Abstract
Matrix-assisted laser desorption–ionization mass spectrometry imaging in transmission-mode geometry (t-MALDI–MSI) can provide molecular information with a pixel size of 1 µm and smaller, which makes this label-free method highly interesting for characterizing the chemical composition of tissues and cells on a (sub)cellular level. However, a major hindrance for wider use of the technology is the reduced ion abundance at small pixel sizes. Here we mitigate this problem by use of laser-induced post-ionization (MALDI-2) and by adapting a t-MALDI-2 ion source to an Orbitrap mass analyzer. We demonstrate the crucial sensitivity and accuracy boosts that are achieved with this combination by visualizing the distribution of numerous phospho- and glycolipids in mouse cerebellum and kidney slices, and in cultured Vero B4 cells. With brain tissue, a pixel size of 600 nm was achieved. Our method could constitute a valuable new tool for research in cell biology and biomedicine.
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Data availability
The data that support the findings of this study, in particular all MSI data as presented in the main text, are available to download in the vendor neutral imzML format from https://uni-muenster.sciebo.de/s/bDrohQ7xJi7ZMIK or from the corresponding author on request. Selected MSI data were also uploaded to the METASPACE platform38 for visualization and annotation (https://metaspace2020.eu/project/Niehaus-2019-Transmission-MALDI-2).
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Acknowledgements
We thank N. Schwab (Institute for Translational Neurology), S. Albrecht (Institute of Neuropathology) and T. Weide (Molecular Necrophology) for providing mouse brain and kidney samples and for help with data interpretation; J. Müthing, N. Skutta, D. Mense for cell culturing; H. Nüsse for SEM images; W. Brock and Tascon GmbH for profilometer measurements; C. Bookmeyer, G. Pohlentz and M. Mormann for assistance with lipid assignments; M. Wiese for programming a software module for steering the piezo stage; A. Korf for expert assistance with MZmine software; W. Kramer (Fotozentrale of the University Hospital Münster) for design and production of Fig. 1; and members of the central fine-mechanical workshop of the Münster Medical School for help building the t-MALDI stage. Financial support by the German Research Foundation (DFG; grants DR 416/12-1, DR 416/13-1, SO 976/3-1 and SO 976/4-1) and the Interdisciplinary Center for Clinical Research (IZFK; grant Drei2/018/17) is gratefully acknowledged.
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M.N., J.S. and K.D. conceived the experiments; M.N. and J.S. designed the t-MALDI ion source; M.B. provided crucial input for the adaptation with the dual-ion funnel injector and the Orbitrap mass analyzer; M.N. and J.S. conducted the experiments; M.N., J.S. and K.D. performed the data analysis; K.D. and J.S. provided funds; and M.N., J.S. and K.D. wrote the paper.
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M.N., J.S. and K. D. declare no competing interests. M.B. is a general manager of Spectroglyph LLC, the company that developed and made commercially available the dual-funnel MALDI–ESI Injector interface.
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Supplementary Figure 1 Overview bright field image of the mouse brain section evaluated in Figs. 2, 4 and Supplementary Fig. 3.
Overview bright field image of the mouse cerebellum tissue section that was used to generate the ion images of Fig. 2, Fig. 4, and Supplementary Fig. 2, respectively. The adjacent areas that were analyzed for producing the ion images are indicated by the black frames. For Fig. 2, the big rectangle to the right denotes the positive ion mode measurements whereas the negative ion mode measurements (left) were conducted on three separate days. The HCCA matrix-coated tissue sample remained in the t-MALDI ion source during the full experimental circle, without that this caused any notable degradation in analytical performance.
Supplementary Figure 2 Comparison of t-MALDI with t-MALDI-2.
(a) t-MALDI (black trace, top panel) and t-MALDI-2 (red trace, bottom) mass spectra acquired from mouse cerebellum in the positive ion mode at 1 µm pixel size. HCCA was used as a matrix. (b) Bright field image of the areas across which the mass spectra were acquired, the microscopic image was taken prior to spray-coating the HCCA MALDI matrix. (c) Ion images of selected lipids acquired in the t-MALDI (top) and t-MALDI-2 modes (bottom). Comparable experiments from four different mouse brain samples yielded similar results.
Supplementary Figure 3 Comparison of [DAG(36:1)]+- and putative PC(36:1)-precursor-derived ion images.
Ion images of four most prominent 36:1-phospholipid ion signals detected from mouse cerebellum by t-MALDI-2 in the positive ion mode and that of the [DAG(36:1)]+ dissociation product. The same data set as used for producing Fig. 2 of the main text was evaluated. (a) m/z 605.552, [DAG(36:1)]+; (b) m/z 703.526, PA(36:1); (c) m/z 729.542, PC(36:1)-N(CH3)3 or isobaric PA(38:2); (d) 746.469; PE(36:1); (d) m/z 788.616, PC(36:1); (f) m/z 790.559, PS(36:1). All ions were detected as [M + H]+ species. All ‘Viridis’ false color pallets were adjusted to optimize the presentation of the individual ion images; hence, they are not to scale if the images were to be compared among each other. Comparable experiments from four different mouse brain samples yielded similar results.
Supplementary Figure 4 MSI and light microscopy data of mouse kidney tissue—part 1 and part 2.
(a) Microscopic image of a 6 µm-thick, H&E-stained section of a mouse kidney tissue. The stain was produced following the t-MALDI measurements and removing the matrix by a washing step. The black rectangular area indicates the approximate regions with which t-MALDI-2–MSI experiments were conducted. (b) Autofluorescence image taken of the analyzed section after the MSI measurement. (c to f) Representative t-MALDI-2–MS images acquired in the positive ion mode: (c) m/z 768.544, PE(38:4)+, (d) m/z 724.524, PE(O-36:5)/PE(P-36:4); (e) m/z 792.555, PE(40:6), (f) m/z 644.502, CerP(36:1-OH; presumably CerP(d18:1/C18:0-)). All ions were detected as [M + H]+ species. (g) Mass spectrum averaged over 580,000 pixels. Only a few selected major ion signals are annotated based on accurate mass. A more complete assignment of the detected lipids is provided in Supplementary Table 3. HCCA was used as the MALDI matrix and prepared using a spraying protocol. The ablation laser was focused to an effective spot size of about 1.3 µm by diameter and the step size of the piezo stage was set to 1.2 µm. Comparable experiments from one different mouse kidney sample yielded similar results.
Supplementary Figure 5 Single pixel MS/MS data recorded at 1 µm pixel size.
(a) Bright-field microscopic image of a 6 µm-thick section of a mouse brain tissue before matrix coating. (b) t-MALDI-2-MS/MS images of diagnostic fragments recorded from the same section following spray-coating with HCCA matrix. (c) Single pixel MS/MS spectrum of GalCer(d18:1/C22:1), m/z of the [M + H]+ precursor, 810.681; (d) MS/MS spectrum of PE(40:6), m/z of the [M + H]+ precursor, 792.554, recorded from 4 adjacent pixels, and (e) MS/MS spectrum of PS(40:6), m/z of the [M + H]+ precursor, 836.543, also recorded from 4 pixel. Experiments were conducted on a single sample only.
Supplementary Figure 6 SEM images of brain sections coated with HCCA matrix before and following t-MALDI-2-MSI.
(a) SEM image of a 6 µm-thick mouse brain tissue section, spray-coated with HCCA matrix according to the protocol outlined in the Methods section. The displayed region corresponds to the white matter of mouse cerebellum. (b) Ablation crater pattern formed during a t-MALDI-2-MSI experiment and use of 25 laser pulses. The t-MALDI-MSI experiment was conducted at a step size of 5.0 µm. (c) Enlarged view into the irradiated sample. Experiments were conducted on a single sample only.
Supplementary Figure 7 Tandem-MS data to demonstrate adduct formation with indium cations.
An example tandem MS spectrum of an (unknown) analyte species with an indium adduct. Experiments were conducted on a single sample only.
Supplementary Figure 8 Bright-field and t-MALDI-2-MSI-data of cultured Vero B4 cells in the negative ion mode.
Bright field and exemplary ion images of a Vero B4 cell culture imaged by t-MALDI-2-MSI in the negative ion mode (cf. Fig. 5 of the main text for positive ion mode measurements). (a) Bright field image of sub-confluently grown cells with the DHB matrix applied by sublimation; the depicted area displays the region from which the ion images in panels b to d were recorded. (b) M/z 742.538, PE(36:2); (c) m/z 788.545, PS(36:1); (d) m/z 861.550, PI(36:2); all ions were detected as [M–H]− species. A more complete list of tentatively annotated lipids is provided in Supplementary Table 4. Comparable experiments from one different mouse kidney sample yielded similar results.
Supplementary Figure 9 Snapshots of the t-MALDI setup.
Snapshots of the custom-build t-MALDI-2 ion source. (a) The following components are depicted: 1- telescope lenses for beam manipulation. One of the lenses is attached to a piezo stage for fine adjustment of the laser focus on the sample slide; 2- dielectric mirror in front of the quartz window guiding the laser beam into the ion source; 3- UV-grade mirrors; 4- focusing lens for the CCD camera. (b) The interior components of the ion source. 1- 50x magnifying UV-grade microscope objective; 2- piezo sample stage; 3- ITO coated slide holder; 4- constant force spring to account for the weight of the attached sample holder and PEEK bracelet.
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Niehaus, M., Soltwisch, J., Belov, M.E. et al. Transmission-mode MALDI-2 mass spectrometry imaging of cells and tissues at subcellular resolution. Nat Methods 16, 925–931 (2019). https://doi.org/10.1038/s41592-019-0536-2
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DOI: https://doi.org/10.1038/s41592-019-0536-2
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